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You should not need 30% PhiX as long as the flow-cell is not being overclustered and your barcodes have good nucleotide diversity. Our sequencing facility usually uses 10% PhiX. It has always worked for us except on one occasion where we submitted samples with very low-diversity barcodes, so I would definitely avoid that. Otherwise, 30% sounds excessive and you might lose on coverage. Do you know if the flow-cells they will be using are patterned?
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Cluster identification is obviously not the problem?
I assume Illumina just ported the X10 software (designed for genomic samples only). The software is one generation behind the one of the Hiseq 2500 and the Miseq and I guess sensitive to overall fluorescence intensity changes?
Originally posted by SNPsaurus View PostI would have thought that having a patterned flowcell would reduce the need for PhiX to discriminate clusters since there should be fewer "almost merged" clusters. Any ideas why there might be more PhiX needed?
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I would have thought that having a patterned flowcell would reduce the need for PhiX to discriminate clusters since there should be fewer "almost merged" clusters. Any ideas why there might be more PhiX needed?
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We typically run ~10% phiX for ddRAD libraries on our HiSeq2500 running v4 chemistry, and they've been running fine. We typically see ~91% PF (%) at ~850 K/mm2 density, ~236 M Reads, ~215 M Reads PF, ~9% alignment to phiX (these are averages from the last three libraries/lanes we've run). I'm sure all ddRAD libraries are not created equal, though. These are from a group with considerable experience making their libraries.
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Originally posted by luc View PostWhich HiSeq model are you running?
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How much phiX to spike in for ddRADseq library on HiSeq?
Our lab is preparing for a large scale ddRADseq project (~3000 samples). In doing the calculations for how many lanes of sequencing we will need to achieve our desired depth of coverage I am finding it difficult to get a consensus answer as to amount of PhiX spiked into a HiSeq lane.
When we spoke with Illumina directly, they recommended we spike 10% PhiX into our final libraries before sequencing. They also said that in the past more PhiX was needed for the older software to correctly identify clusters. When we talked to a sequencing provider they stated that they spike in 30% PhiX for ddRADseq libraries. This seems like a big discrepancy to me.
For folks with recent ddRAD experience, how much PhiX did you spike into your library?
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